单核细胞增生性李斯特菌分子生物学检测技术的研究进展

单核细胞增生性李斯特菌(Listeria monocytogenes,LM)是主要食源性致病菌之一,可引起李斯特菌病,感染严重者会出现致死现象。传统的单增李斯特菌检测方法耗时长,步骤繁琐。因此,特异性强,高效性以及简便的检测手段已成为研究热点。本文综述了运用分子生物学手段对单核细胞增生性李斯特菌检测的研究概况,并对该技术未来发展趋势进行了展望。      

Comparison of 3M Petrifilm environmental Listeria plates against standard enrichment methods for the detection of Listeria monocytogenes of epidemiological significance from environmental surfaces

ABSTRACT:  Environmental monitoring using sensitive methods for detection and elimination of harborage sites of Listeria monocytogenes is key to the control of this organism. The 3M™ Petrifilm™ Environmental Listeria (EL) Plate—a no enrichment method—was compared with the USDA/FSIS, modified USDA/FSIS (mUSDA), and ISO methods for detection/recovery of L. monocytogenes on 4 environmental surfaces (brick, dairy board, stainless steel, and epoxy resin). The efficacy of 3 sampling devices including the Microbial-Vac system^®, environmental sponge, and 3M Quick swab in recovering epidemiologically significant strains of uninjured and sublethally injured L. monocytogenes from environmental surfaces was evaluated. Environmental surfaces were inoculated with Listeria to obtain final cell densities of approximately 10 to 100 CFU/100 cm². The surfaces were then sampled and processed. For all methods, percent recovery (% samples where Listeria was detected) was significantly higher ( P < 0.05) for uninjured cells (75% to 100%) compared to injured cells (58.9% to 81.1%). The Petrifilm EL Plate method efficiently recovered both low level and injured Listeria populations from environmental test surfaces when used in conjunction with environmental sponge and the 3M Quick swab sampling. The mUSDA method was superior to all other methods for recovering both uninjured (100% recovery) and injured L. monocytogenes (80.8% to 81.1% recovery). Sponges and swabs were equally effective in recovering uninjured and injured Listeria and were significantly different ( P < 0.05) from the Microbial-Vac system. The findings indicate that both mUSDA and Petrifilm EL Plate methods can be used for the detection of potentially injured Listeria on food processing environmental surfaces.     

A comparative study of the 'FDA' and 'USDA' methods for the detection of Listeria monocytogenes in foods

Nineteen laboratories across Canada took part in a comparative study of the 'FDA' and 'USDA' methods for the detection of Listeria monocytogenes in foods and environmental samples. The results show that the enrichment period of the FDA method can be shortened from 7 to 2 days without substantially reducing the number of positive samples. With a limited number of samples, the USDA method proved to be slightly more efficient in isolating L. monocytogenes than the FDA method. Fraser broth, in principle, proved to be useful as a screening tool but is not very selective. Oxford agar and lithium chloride-phenylethanol-moxalactam medium were better than modified McBride's agar in isolating this microorganism.     

Listeria monocytogenes virulence and pathogenicity,a food safety perspective

Several virulence factors of Listeria monocytogenes have been identified and extensively characterized at the molecular and cell biologic levels, including the hemolysin (listeriolysin O), two distinct phospholipases, a protein (ActA), several internalins, and others. Their study has yielded an impressive amount of information on the mechanisms employed by this facultative intracellular pathogen to interact with mammalian host cells, escape the host cell's killing mechanisms, and spread from one infected cell to others. In addition, several molecular subtyping tools have been developed to facilitate the detection of different strain types and lineages of the pathogen, including those implicated in common-source outbreaks of the disease. Despite these spectacular gains in knowledge, the virulence of L. monocytogenes as a foodborne pathogen remains poorly understood. The available pathogenesis and subtyping data generally fail to provide adequate insight about the virulence of field isolates and the likelihood that a given strain will cause illness. Possible mechanisms for the apparent prevalence of three serotypes (1/2a, 1/2b, and 4b) in human foodborne illness remain unidentified. The propensity of certain strain lineages (epidemic clones) to be implicated in common-source outbreaks and the prevalence of serotype 4b among epidemic-associated stains also remain poorly understood. This review first discusses current progress in understanding the general features of virulence and pathogenesis of L. monocytogenes. Emphasis is then placed on areas of special relevance to the organism's involvement in human foodborne illness, including (i) the relative prevalence of different serotypes and serotype-specific features and genetic markers; (ii) the ability of the organism to respond to environmental stresses of relevance to the food industry (cold, salt, iron depletion, and acid); (iii) the specific features of the major known epidemic-associated lineages; and (iv) the possible reservoirs of the organism in animals and the environment and the pronounced impact of environmental contamination in the food processing facilities. Finally, a discussion is provided on the perceived areas of special need for future research of relevance to food safety, including (i) theoretical modeling studies of niche complexity and contamination in the food processing facilities; (ii) strain databases for comprehensive molecular typing; and (iii) contributions from genomic and proteomic tools, including DNA microarrays for genotyping and expression signatures. Virulence-related genomic and proteomic signatures are expected to emerge from analysis of the genomes at the global level, with the support of adequate epidemiologic data and access to relevant strains.     

PMA-LAMP检测单增李斯特活菌方法的建立

建立一种将荧光染料Propidium Monoazide(PMA)与环介导等温扩增(LAMP)相结合的检测方法,用于高效检测活的单核细胞增多性李斯特氏菌(简称单增李斯特菌)。利用PMA抑制单增李斯特死菌后进行LAMP扩增实验、并研究了PMA-LAMP方法检测单增李斯特活菌的灵敏度,同时与PMA-PCR方法灵敏度进行比较。结果表明,50μmol/L的PMA处理浓度为5×108cfu/mL单增李斯特死菌,能够完全抑制LAMP扩增。PMA-LAMP方法检测单增李斯特活菌的检出限为4.9×101cfu/mL,其灵敏度是PMA-PCR方法的10倍。该方法可以作为一种快速检测单增李斯特活菌的新技术。     

食品中单增李斯特氏菌检测PCR-免疫胶体金 试纸条方法的建立

目的 建立食品中单核增生李斯特氏菌快速检测PCR-免疫胶体金试纸条法。方法 通过设计特异性引物建立单增李斯特氏菌检测PCR方法并使用免疫胶体金技术建立PCR产物快速检测试纸条; 用试验菌株检测PCR-免疫胶体金试纸条方法的检测特异度与敏感度。使用新建方法对市售肉制品和乳制品中单核增生李斯特氏菌进行检测, 验证该方法在食品检测中的可行性。结果 PCR-免疫胶体金法具有良好的特异度, 敏感度比标准琼脂糖凝胶电泳法高100倍。采集乳品样品131份, 阳性样品1份, 检出率1.53%; 肉制品224份, 阳性样品4份, 检测率1.79%。结论 建立的单增李斯特氏菌检测PCR-免疫胶体金试纸条法特异度好, 敏感度高, 适用于食品中单增李斯特氏菌的检测。     

Bayesian synthesis of a pathogen growth model: Listeria monocytogenes under competition

The Bayesian synthesis method is applied to data from two studies of Listeria monocytogenes grown in broth monocultures to draw inferences about the joint distribution of two Baranyi growth model parameters-lag time and maximum specific growth rate. The resultant joint distribution is then combined with prior distributions for the initial and maximum pathogen density parameters under competitive growth conditions. Finally, the pathogen growth model is updated using the Sampling/Importance Resampling (SIR) algorithm with data on L. monocytogenes growth in competition with natural microflora in fish. Although the latter data provide no information on the stationary phase to directly estimate the maximum pathogen density parameter, combining them with relevant prior information provides a means to characterize L. monocytogenes growth in a food with mixed microbial populations. Based on a specified tolerance for L. monocytogenes growth, the updated model provides a storage time limit for fish held at 5 degrees C, pH 6.8, 43% CO(2), 57% N(2).     

FTA滤膜用于PCR检测单核细胞增生李斯特氏菌的研究

建立单核细胞增生李斯特氏菌(Listeria moncytones,LM)快速、敏感、特异的PCR检测方法.利用FTA滤膜提取模板DNA,采用PCR特异性扩增单增李斯特菌的溶血素基因(HIyA),并评价该方法的特异性与灵敏性.引物能特异性的扩增单增李斯特的HIyA基因,而其他细菌的扩增结果均呈现阴性:利用FTA滤膜提取模板直接检测单增李斯特具有较高的灵敏度,灵敏度为l 02 cfu/mL.利用FFA滤膜提取模板,操作简便,成本低且具有较高的灵敏度,为食品中单核细胞增生李斯特氏菌的快速检测提供新的手段.     

食品中单核细胞增多李斯特菌的快速检测

单核细胞增多李斯特菌是一种能引起人畜共患病和食源性疾病的致病菌。本文简述了单增李斯特菌的特性和毒力因子,介绍了从分子生物学和免疫学发展起来的核酸探针杂交、PCR、ELISA、免疫传感器等快速检测方法。这些快速检测方法与传统检测方法相比不仅缩短了检测时间,提高了检测效率,还提高了检测方法的灵敏度和特异性,对于单增李斯特菌的检测具有良好的应用前景。      

The VIT technology for rapid detection of Listeria monocytogenes and other Listeria spp

Detection of Listeria monocytogenes is generally performed in a two-step cultural enrichment process and takes on average 1 week until the biochemical identification of a L. monocytogenes suspicious colony is completed. However, food processing companies depend increasingly on test methods, which attempt to generate results comparable to standard methods but in reduced time-frame and which allow to release produced batches dependent on such results. In the present study, the vermicon identification technology (VIT), a rapid commercial test system using fluorescently labelled gene probes, was compared to a cultural standard method. In total, 298 naturally contaminated samples were analysed. The sensitivity and the specificity of the VIT system were 100% for the detection of L. monocytogenes and 97.1% and 100%, respectively, for the detection of the genus Listeria.     

单增李斯特菌胶体金免疫层析试纸条的研制

以单增李斯特菌(LM)内化素A蛋白(InlA)单克隆抗体为基础,研制其胶体金免疫层析检测试纸条。方法 采用DNAStar软件对LM inlA全长基因编码蛋白进行抗原表位分析,截取部分inlA基因片段构建原核表达质粒,诱导表达和纯化获得重组蛋白。以该蛋白免疫BALB/c小鼠,筛选高效分泌抗InlA单克隆抗体的杂交瘤细胞株,制备单克隆抗体;以双抗体夹心的原理研制胶体金免疫层析检测试纸条,并对其特异性、敏感性、稳定性进行评价。结果 筛选到2株高效分泌抗InlA单克隆抗体的杂交瘤细胞株,抗体属于IgG1亚类,小鼠腹水抗体效价为1∶64000;研制的试纸条可与LM发生阳性反应,而与非LM李斯特菌、链球菌、鼠伤寒沙门菌、大肠杆菌O157∶H7等食源性致病菌均不发生阳性反应;LM纯培养物敏感性为2.4×10^5cfu/ml,模拟猪肉样品敏感性为4.0×10⁶ cfu/ml;4℃保存期可达16周以上。结论 研制的胶体金免疫层析试纸条具有快速、特异、敏感等优点,可以用于样品中LM的快速检测。     

Analysis of PCR-based methods for characterization of Listeria monocytogenes strains isolated from different sources

Listeria monocytogenes strains, isolated from various sources (food, environment, and animals), were used to test different PCR-based methods to investigate their capability to define the strain origin. RAPD-PCR with three primers and the SAU-PCR method, in which the DNA was first digested with the Sau3A restriction endonuclease and then amplified with a primer designed on the restriction site, were carried out, and the profiles obtained were used to perform cluster analysis. Based on the cluster analysis of Listeria spp. strains, obtained from international collections, the coefficient of similarity was selected. The results obtained showed that the methods tested in the study gave different levels of differentiation between the strains tested. The RAPD protocol using the P1254 primer and the SAU-PCR gave appreciable results only for strains isolated from animals and from a food processing plant in two different periods of the year 2003. Better differentiation was observed using the RAPD-PCR with primer D8635. As a matter of fact, it was able to distinguish L. monocytogenes obtained from different species of animals, different food samples and strains from the same production plant isolated in different periods of the year. Also primer M13 gave positive results, but the coefficient of similarity to use had to be increased to 80%. On the basis of the results observed, RAPD-PCR with primers D8635 and M13 should be considered reliable tools for epidemiological investigations focusing on L. monocytogenes.     

基于双启动引物特异性检测单核细胞增生李斯特氏菌的PCR方法

以单核细胞增生李斯特氏菌iap基因为靶基因,利用一新型PCR引物设计方法--双启动引物（Dual-priming oligonucleotide,DPO）,建立了特异性检测单核细胞增生李斯特氏菌的DPO-PCR方法,测试了DPO-PCR方法退火温度不敏感性、特异性及灵敏度,并在实践检测中进行了初步应用。结果显示:该方法检测单核细胞增生李斯特氏菌的灵敏度为1.51×102CFU/mL;退火温度不敏感性测试中,与常规PCR引物相比,DPO引物在48⁶8℃退火温度范围内均能够高效率地扩增靶基因;特异性测试中,DPO-PCR方法能特异地检测出目标菌,与其他菌株无非特异性扩增反应,比常规PCR方法显示出更强的特异性。实践应用证明,利用DPO-PCR方法对130份样本进行检测,共计检出9份单核细胞增生李斯特氏菌阳性样本,经国标法（GB/T 4789.30-2008）复检,两者检测结果一致,显示出良好的实用性,为单核细胞增生李斯特氏菌的快速准确检测提供了新方法。      

食源性致病菌单增李斯特菌检测技术的研究进展

单增李斯特菌是一种兼性厌氧性食源性致病菌,对低温、高盐及消毒剂的抵抗力很强,感染后可能产生低热、高热或其他全身性疾病,免疫力低下的人可能会引起肠胃炎、孕妇流产、早产或死产,甚至会产生脑膜炎。LM的传统检测方法是先进行增菌,再经过氧化氢酶试验、溶血试验、血清学试验等进行鉴定,操作性强、灵敏度高、成本低,但是检测周期长达7 d,无法对目标食物进行快速检测。本文综述了振动光谱学检测方法、免疫学检测方法、分子生物学检测方法、代谢组学检测法、生物传感器等食源性单增李斯特菌的检测方法,并比较其优缺点,以期为食品中LM的快速检测方法的研究提供参考。     

Preparation of Listeria monocytogenes specimens for molecular detection and identification

Listeria monocytogenes is a common foodborne pathogen that has the capacity to cause severe clinical illness in vulnerable human population groups. The availability of rapid and specific laboratory tests to identify this bacterium is essential for preventing an otherwise easily treated malaise from developing into a life-threatening disease. To this end, a variety of rapid, sensitive and precise nucleic acid-based assays have been developed, contributing to the improved diagnosis of listeriosis. Nonetheless, since many molecular assays rely on enzymatic reaction for template amplification, which is liable to interference from inhibitory substances present in clinical, food and environmental specimens, they often require purified nucleic acids as starting material for test consistency. As a consequence, considerable efforts have been directed toward the development of innovative and efficient sample handling procedures that reduce and eliminate inhibitory elements present in the specimens. By reviewing the recent progresses in the sample preparation methods that have been described for enhanced molecular detection and identification of L. monocytogenes, including rapid procedures for cultured isolates, more elaborate techniques for processing clinical, food and environmental samples, and specific considerations in preparing samples for quantitative PCR analysis, this article highlights further research requirement in the specimen processing protocols that form the basis for continued improvement in the overall performance of molecular assays for listeriosis.     

双重荧光定量PCR检测沙门菌和单核细胞增生李斯特菌方法的建立

目的建立双重荧光定量PCR方法,快速检测沙门菌和单核细胞增生李斯特菌。方法通过设计特异性引物和探针,扩增沙门菌的fimY基因和单核细胞增生李斯特菌的hly基因,采用倍比梯度稀释法检测该体系的灵敏度,以另外7株肠道致病菌评价检测体系的特异性;建立了沙门菌和单核细胞增生李斯特菌感染小鼠的检测模型以验证方法的适用性。结果建立了同时检测沙门菌和单核细胞增生李斯特菌的双重荧光定量PCR方法,从DNA提取到检测完毕仅需2.5 h。检测两种病原菌的灵敏度分别为11和12.8 copies/μl,特异性为100%,符合率为93.3%。结论该法缩短了检测时间,并有良好的灵敏性和特异性,在疾病防控及食品卫生行业中很有应用前景。     

单增李斯特菌鞭毛蛋白提取方法的研究

本实验对单增李斯特菌鞭毛蛋白提取方法进行研究,分别在23℃和37℃的条件下对单增李斯特菌(血清型IVb)进行扩增培养,发现23℃下单增李斯特菌产鞭毛的能力更强。运用酸解法处理单增李斯特菌后,分别通过超速离心法和硫酸铵沉淀法对鞭毛蛋白进行纯化,SDS-PAGE 电泳以及电镜的实验结果表明,超速离心较硫酸铵沉淀法简便、耗时短、纯度高、产量高,适用于单增李斯特菌鞭毛蛋白的提取。     

RapidChek检测食品中单增李斯特菌的方法评价

目的评价RapidChek法检测食品中单增李斯特菌的检测效果并验证。方法采用t检验,比较RapidChek方法与GB 4789.30-2016方法的培养基增菌效果。依据ISO 16140:2003《食品和动物饲料微生物学-可替代方法的验证方案》,比较RapidChek检测方法与GB 4789.30-2016检测方法的检测效果,涉及的性能指标有相对准确性、相对特异性和相对灵敏度、包含性和排他性。结果 RapidChek检测方法增菌培养基效果优于GB 4789.30-2016方法增菌培养基LB_1。根据RapidChek检测方法、GB 4789.30-2016培养基+RapidChek试纸条方法、RapidChek培养基+GB 4789.30分离鉴定方法的统计检验得出,3种方法与参照方法在相对准确性、相对特异性和相对灵敏度方面无显著性差异。在包含性和排他性方面,RapidChek检测方法与GB 4789.30-2016检测方法的检测结果均一致。结论在所验证的指标上,RapidChek检测方法(包括与GB4789.30-2016组合的方法)与GB 4789.30-2016方法无差异。     

免疫磁分离技术在食源性单增李斯特菌检测中应用的研究进展

食源性单增李斯特菌是李斯特菌属中的唯一能引起人类疾病的病原菌,致死率30%~70%,并严重威胁着人类健康。早期快速准确地检测出食品中可能污染的单增李斯特菌对于减少死亡率非常重要,因此亟需建立一些快速、灵敏和高特异性的检测方法。现有单增李斯特菌的检测方法对未经前增菌的食品样本检测灵敏度较低,限制了这些方法直接用于食品样本中单增李斯特菌的快速检测。免疫磁分离是一种可以短时间内高效富集样本中目的菌的技术,与常用的检测方法结合,可以缩短检测周期,提高检测灵敏度。本文综述了免疫磁分离技术在食源性单核细胞增生性李斯特检测中应用的研究进展。      

单核增生李斯特氏菌近红外快检方法建立与应用

目的建立一种近红外荧光免疫法快速检测单增李斯特氏菌的方法。方法采用近红外荧光染料Dylight800标记单增李斯特菌单克隆抗体,结合免疫侧向流技术制备单增李斯特菌快速检测试纸条。结果整个实验过程仅需45 min,对食品中单增李斯特氏菌最低检测限为500 CFU/mL,与其他5种食源性致病菌均无交叉反应。特异性为89.47%,敏感性为100%。采用近红外荧光免疫层析法和传统方法对30份食品进行检测,结果发现2种方法符合性达93.3%。结论所研制的单增李斯特菌的近红外快检试纸条具有特异性、敏感性较高的特点,适用于食品样本中单增李斯特菌的即时检测。